Latest revision as of 23:10, 28 September 2011

pGA vector Assay

Prepare these mixtures on ice

Obtain a 40 uL aliquot of BL21 cells.
Add 120 uL of ice water to the aliquot.
The total volume is now 160 uL; split evenly among four labeled tubes: INS + BCK, INS + BCK, INSctrl, BCKctrl.
- INS + BCK tubes (x 2)
  - add 1 uL of 10X pGA Gibson product (1A3 BCK/INS pLacGFP)
- INSctrl tube
  - add 100 pg of pLacGFP gel extract
- BCKctrl
  - add 100 pg of 1A3 gel extract
Repeat steps 1-3 for the comparison vector pSB using the following instead:
- 1 uL of pSB Gibson product (T19-1A3/pLacGFP)
- 1 ng INS (pLacGFP- gel extract)
- 1 ng BCK (T19-1A3- gel extract)
Once all the samples are ready, begin the transformation.
- Rescue each sample in 500 mLs of LB
- Incubate all samples @ 37oC for ~45 min.
Plate 50 uL on each sample onto a LB + Chlor + Amp + IPTG plate.
- 1 plate for each control in each vector set.
- 3 plates for each Gibson product tube in each set. ( 6 plates for each vector set + 2 control plates)

@@ Line 1: / Line 1: @@
 {{Template:Team:Washington/Templates/Top}}
-=pGA Vector Assay=
-.	Prepare stocks for protease inhibitor, DNAse, and lysozyme.
+=pGA vector Assay=
-*a.	Protease Inhibitor = 25x stock ; one tablet into 2ml of buffer
-*b.	DNAses = 100x stock (10mg/ml initial → 0.1mg/mL final)
+*Prepare these mixtures on ice
-*c.	Lysozyme = 10x stock (10mg/ml initial → 1mg/mL final)
+# Obtain a 40 uL aliquot of BL21 cells.
-.	Resuspend 50ml of each type of cell culture in 1ml of this mixture: 850ul sodium phosphate buffer, 40ul protease inhibitor, 10ul DNAse (0.1mg/ml final), and 100ul lysozyme (1mg/ml final).If testing multiple reactions, just multiply the volumes and divide into eppendorf tubes so that each reaction gets 1mL of cell suspension.
+# Add 120 uL of ice water to the aliquot.
-*a.	Buffer: 1ml = 1000ul - (40+10+100) → 850ul
+# The total volume is now 160 uL; split evenly among four labeled tubes: INS + BCK, INS + BCK, INSctrl, BCKctrl.
-*b.	Protease inhibitor: 25x (xml) = 1x (1ml) → 40ul
+#* INS + BCK tubes (x 2)
-*c.	DNAses: (10mg/ml)Xul = (0.1mg/ml)1ml  → 10ul
+#** add 1 uL of 10X pGA Gibson product (1A3 BCK/INS pLacGFP)
-*d.	Lysozyme: (1mg/ml)Xul = (1mg/ml) 1ml → 100ul
+#* INSctrl tube
-.	To lyse cells, add 111uL 10% triton (1% final) and mix the tube at room temperature for 30 min. Then, centrifuge the tubes at max. speed for 15 min (or until the liquid is very clear and not cloudy.
+#** add 100 pg of pLacGFP gel extract
-*x/(1000 +x) = 1/10  ….................. x = 111ul
+#* BCKctrl
-.	Transfer the liquid on top to new labeled eppendorf tube (leave the pellet of lysed stuff; our protein should be sufficiently soluble in aqueous solutions), tube perhaps containing master mix to initiate reaction.
+#** add 100 pg of 1A3 gel extract
-.	Place Target polyspring inserts into the Target DP glass vials.
+#Repeat steps 1-3 for the comparison vector pSB using the following instead:
-.	Cell Lysis
+#* 1 uL of pSB Gibson product (T19-1A3/pLacGFP)
-*a.	Sonicate --use micro tip, 60%, 30 on 30 off (POST-assay: cell lysate not so effective)
+#* 1 ng INS (pLacGFP- gel extract)
-*b.	Bugbuster --Use 10x bugbuster, follow protocol (POST-assay: cell lysate not so effective)
+#* 1 ng BCK (T19-1A3- gel extract)
-*c.	Triton X-100 --Use 1% triton (POST-assay: most effective for cell lysate)
+#Once all the samples are ready, begin the [https://2011.igem.org/Team:Washington/Protocols/Elect. transformation].
+#* Rescue each sample in 500 mLs of LB
+#*Incubate all samples @ 37oC for ~45 min.
+#Plate 50 uL on each sample onto a LB + Chlor + Amp + IPTG plate.
+#*1 plate for each control in each vector set.
+#*3 plates for ''each'' Gibson product tube in each set. ( 6 plates for each vector set + 2 control plates)

Team:Washington/Protocols/pGA.

From 2011.igem.org

Latest revision as of 23:10, 28 September 2011

pGA vector Assay